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单细胞鉴定法鉴定包含二硫键的蛋白质的自动转运蛋白介导的大肠杆菌表面展示。

Single-cell characterization of autotransporter-mediated Escherichia coli surface display of disulfide bond-containing proteins.

机构信息

Department of Chemical and Biomolecular Engineering, University of Houston, Houston, Texas 77204, USA.

出版信息

J Biol Chem. 2012 Nov 9;287(46):38580-9. doi: 10.1074/jbc.M112.388199. Epub 2012 Sep 27.

Abstract

Autotransporters (ATs) are a family of bacterial proteins containing a C-terminal β-barrel-forming domain that facilitates the translocation of N-terminal passenger domain whose functions range from adhesion to proteolysis. Genetic replacement of the native passenger domain with heterologous proteins is an attractive strategy not only for applications such as biocatalysis, live-cell vaccines, and protein engineering but also for gaining mechanistic insights toward understanding AT translocation. The ability of ATs to efficiently display functional recombinant proteins containing multiple disulfides has remained largely controversial. By employing high-throughput single-cell flow cytometry, we have systematically investigated the ability of the Escherichia coli AT Antigen 43 (Ag43) to display two different recombinant reporter proteins, a single-chain antibody (M18 scFv) that contains two disulfides and chymotrypsin that contains four disulfides, by varying the signal peptide and deleting the different domains of the native protein. Our results indicate that only the C-terminal β-barrel and the threaded α-helix are essential for efficient surface display of functional recombinant proteins containing multiple disulfides. These results imply that there are no inherent constraints for functional translocation and display of disulfide bond-containing proteins mediated by the AT system and should open new avenues for protein display and engineering.

摘要

自动转运蛋白(ATs)是一类含有 C 端β桶形成结构域的细菌蛋白,该结构域有助于 N 端的过客结构域的易位,过客结构域的功能范围从粘附到蛋白水解。用异源蛋白替换天然过客结构域是一种很有吸引力的策略,不仅可用于生物催化、活细胞疫苗和蛋白质工程等应用,还可用于深入了解 AT 易位的机制。AT 有效地展示含有多个二硫键的功能重组蛋白的能力在很大程度上仍存在争议。通过采用高通量单细胞流式细胞术,我们系统地研究了大肠杆菌 AT 抗原 43(Ag43)展示两种不同重组报告蛋白的能力,这两种重组报告蛋白为含有两个二硫键的单链抗体(M18 scFv)和含有四个二硫键的胰凝乳蛋白酶,通过改变信号肽并删除天然蛋白的不同结构域。我们的结果表明,只有 C 端β桶和穿线的α螺旋对于含有多个二硫键的功能重组蛋白的高效表面展示是必需的。这些结果表明,AT 系统介导的含二硫键蛋白的功能易位和展示不存在固有限制,应该为蛋白质展示和工程开辟新途径。

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